7L4S
Crystal structure of the OxyR regulatory domain of Shewanella oneidensis MR-1, reduced form
Summary for 7L4S
| Entry DOI | 10.2210/pdb7l4s/pdb |
| Descriptor | Transcriptional regulator of oxidative stress OxyR (2 entities in total) |
| Functional Keywords | oxyr, dna binding protein |
| Biological source | Shewanella oneidensis |
| Total number of polymer chains | 6 |
| Total formula weight | 202871.74 |
| Authors | |
| Primary citation | Sun, W.,Fan, Y.,Wan, F.,Tao, Y.J.,Gao, H. Functional Irreplaceability of Escherichia coli and Shewanella oneidensis OxyRs Is Critically Determined by Intrinsic Differences in Oligomerization. Mbio, 13:e0349721-e0349721, 2022 Cited by PubMed Abstract: LysR-type transcriptional regulators (LTTRs), which function in diverse biological processes in prokaryotes, are composed of a conserved structure with an N-terminal DNA-binding domain (DBD) and a C-terminal signal-sensing regulatory domain (RD). LTTRs that sense and respond to the same signal are often functionally exchangeable in bacterial species across wide phyla, but this phenomenon has not been demonstrated for the HO-sensing and -responding OxyRs. Here, we systematically examined the biochemical and structural determinants differentiating activator-only OxyRs from dual-activity ones by comparing OxyRs from two , Escherichia coli and Shewanella oneidensis. Our data show that OxyR could function as neither an activator nor a repressor in S. oneidensis. Using OxyR-based OxyR chimeras and mutants, we demonstrated that residues 283 to 289, which form the first half of the last C-terminal α-helix (α10), are critical for the proper function of OxyR and cannot be replaced with the OxyR counterpart. Crystal structural analysis reveals that α10 is important for the oligomerization of OxyR, which, unlike OxyR, forms several high-order oligomers upon DNA binding. As the mechanisms of OxyR oligomerization vary substantially among bacterial species, our findings underscore the importance of subtle structural features in determining regulatory activities of structurally similar proteins descending from a common ancestor. Evolution may drive homologous proteins to be functionally nonexchangeable in different organisms. However, much is unknown about the mechanisms underlying this phenomenon beyond amino acid substitutions. Here, we systematically examined the biochemical and structural determinants differentiating functionally nonexchangeable OxyRs, HO-responding transcriptional regulators from two , Escherichia coli and Shewanella oneidensis. Using OxyR-based OxyR chimeras and mutants, we demonstrated that residues 283 to 289, which form the first half of the last C-terminal α-helix (α10), are critical for the proper function of OxyR and cannot be replaced with the OxyR counterpart. Crystal structural analysis reveals that this last helix is critical for formation of high-order oligomers upon DNA binding, a phenomenon not observed with OxyR. Our findings provide a new dimension to differences in sequence and structural features among bacterial species in determining regulatory activities of homologous regulators. PubMed: 35073744DOI: 10.1128/mbio.03497-21 PDB entries with the same primary citation |
| Experimental method | X-RAY DIFFRACTION (2.4 Å) |
Structure validation
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